张钰付亮鲁超锁涛宋陆军△.原代小鼠肝脏细胞的高效分离纯化与培养*[J].,2014,14(6):1005-1008 |
原代小鼠肝脏细胞的高效分离纯化与培养* |
Isolation,Purification and Primary Culture of Mouse Hepatocyteswith High Viability* |
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DOI: |
中文关键词: 肝脏细胞 原代细胞培养 分离 纯化 小鼠 |
英文关键词: Hepatocytes Primary cell culture Isolation Purification Mouse |
基金项目:上海市科学技术委员会基金项目(09ZR1405900) |
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中文摘要: |
摘要目的:建立一种能稳定获得高活力和高纯度原代小鼠肝脏细胞的分离、纯化及培养方法。方法:应用改良的Seglen 二步法原
位灌注和机械离心分离肝脏细胞,并用改良的高糖DMEM培养基进行培养。台盼蓝拒染法检测接种时肝脏细胞的存活率,倒置
显微镜动态观察肝脏细胞形态变化,应用免疫荧光技术对肝脏细胞进行Albumin 染色。结果:每只小鼠可获取肝脏细胞的总产量
平均为1.35× 106 / g体重,肝脏细胞存活率> 90%。倒置显微镜下观察贴壁前肝细胞直径为35.14 滋m± 4.35 滋m,肝脏细胞在接种
后3 h基本完成贴壁;肝脏细胞接种后24h,所有肝脏细胞均强阳性表达成熟肝脏细胞标志物Albumin,肝细胞纯度> 95%。结
论:改良的分离纯化及培养方法能稳定获得高产量、高活率及高纯度的小鼠肝脏细胞。 |
英文摘要: |
ABSTRACT Objective:A stable method was established for isolation and primary culture of mouse hepatocytes with high purity
and viability. Methods:The C57BL/6 mouse hepatocytes were isolated by a modified two-step collagenase perfusion and low-speed
mechanical centrifugation. The hepatocytes were cultured in modified DMEM with high level of glucose. The viabilities of cells were
evaluated by Trypan blue exclusion before cells were seeded. Cellular morphological changes were observed using a phase contrast
microscopy. The Albumin and CKl9 staining were performed on hepatocytes by immunofluorescence. Results:The total cell yield of
hepatocytes was 1.35× 106 cells/g wet weight. Total cell viability was more than 90%. The diameter of hepatocytes was 35.14 滋m± 4.35
滋m before adherence. The hepatocytes with enlarged and flattened round shape were attached to the surface of collagen-coated dishes 3
hours after seeding. Albumin was positively expressed in all hepatocytes at 24 h after attachment, and the purity of hepatocytes was more
than 95%.Conclusion: Mouse hepatocytes with high quantity, purity and survival rate were obtained by the improved method for
isolation, purification and culture. |
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